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1.
Forensic Sci Int ; 113(1-3): 113-8, 2000 Sep 11.
Article in English | MEDLINE | ID: mdl-10978611

ABSTRACT

Sequencing of mtDNA is an advanced method for the individualisation of traces. Disadvantages of this method are expensive and time-consuming analysis and evaluation procedures as well as the necessary stock of population-genetic data which is still insufficient. Central European institutes of forensic medicine from Germany, Austria, and Switzerland have been working together since the beginning of 1998 to establish a mtDNA database. The aim is to build up a large stock of forensically established data and provide population-genetic data for frequency investigations, which will serve as a basis for expert opinions and scientific research. Good data quality is ensured by using original sequences only. Ring tests, which have been conducted to enhance analytical reliability, revealed a high correspondence rate of the analytical results obtained by the individual member institutes. Today 1410 sequences are available for comparison, of which 1285 sequences in the HV1 and HV2 regions cover the full ranges from 16051 to 16365 and from 73 to 340 (according to Anderson). The major part is formed by Central European sequences comprising 1256 data sets from Germany, Austria, and Switzerland. Today the database contains sequences from a total of 12 European, six African and three Asian countries including 100 sequences from Japan. This paper is aimed at discussing the individualisation potentials of mtDNA as well as the possibilities and limits of ethnic differentiation by means of pairwise sequence differences on the basis of the data stock available.


Subject(s)
Complementarity Determining Regions/genetics , DNA Fingerprinting/methods , DNA, Mitochondrial/genetics , Databases, Factual , Ethnicity/genetics , Forensic Anthropology/methods , Gene Frequency/genetics , Sequence Analysis, DNA/methods , Austria , Genetic Variation/genetics , Germany , Humans , International Cooperation , Japan , Sampling Studies , Switzerland
2.
Forensic Sci Int ; 55(1): 45-58, 1992 Jul.
Article in English | MEDLINE | ID: mdl-1511938

ABSTRACT

A collaborative study using the multilocus minisatellite DNA probe MZ 1.3 was carried out to investigate segregation information, mutation rate, DNA fragment frequencies as well as band sharing characteristics. The fingerprint patterns of 393 children as well as 694 unrelated individuals were analysed after digestion of DNA with the restriction enzyme HinfI. A mutation rate of 1% per meiosis or 0.04% per band was found with a mean number of 26 bands/individual. It was shown that maternal and paternal fragments are inherited in equal proportions. Population frequencies of restriction fragments demonstrated a distribution with increasing frequencies in the small fragment size range below 10 kb as well as the absence of very common or very rare fragments. Our data can be used to calculate simple exclusion probabilities based on the number of non-maternal bands in the child.


Subject(s)
Biometry/methods , DNA Fingerprinting , Paternity , Child , DNA Probes , Data Interpretation, Statistical , Female , Humans , Male , Probability
3.
Forensic Sci Int ; 46(1-2): 11-4, 1990.
Article in English | MEDLINE | ID: mdl-2210538

ABSTRACT

Fingernail specimens with adherent nail-bed were taken from autopsy material with blood groups A, AB, B and O. Frozen 4-5-microns sections were submerged and floated carefully during each working step. Portions of fingernails were contaminated with blood and buccal cells, respectively. Furthermore, fingernail fragments of 8 volunteers were embedded in a biocomponent adhesive according to Grieve and Kotowski (Forensic Sci. Soc., 26 29-34) (1986) and cut by the usual microtome technique. APAAP staining is a proper method for demonstrating blood group antigens in fingernails from groove to margin. Frozen sections as well as smallest specimen embedded in a suitable adhesive are applicable for staining procedures. Using freshly prepared artificial stains, blood group constellations of red blood cells and/or buccal cells adherent on the surface of fingernails may be distinguished from the nail matrix.


Subject(s)
ABO Blood-Group System/immunology , Isoantigens/analysis , Nails/immunology , Humans , Immunoenzyme Techniques
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